Diagnostic test for Collie Eye Anomaly

ABSTRACT

The invention relates to a method for identifying dogs which are genetically normal, heterozygous for, or homozygous for the mutation primarily responsible for Collie eye anomaly (CEA). The method comprises the steps of obtaining a biological sample from a dog and testing DNA in the biological sample for the presence or absence of a 7.8 kilobase deletion within chromosome 37 in which the CEA mutation is located. No deletion is indicative of a normal dog. A deletion on one allele of chromosome 37 is indicative of a dog that is heterozygous for the CEA mutation. A deletion in both alleles of chromosome 37 are indicative of a dog that is homozygous for the CEA mutation. Also provided is a kit for identifying a dog as normal, heterozygous for, or homozygous for the CEA mutation.

This application is a divisional application of U.S. patent application Ser. No. 11/255,019, filed Oct. 20, 2005, now U.S. Pat. No. 7,462,455 which in turn claims priority to U.S. provisional application Ser. No. 60/620,547, filed Oct. 20, 2004, the disclosures of each of which are incorporated herein by reference.

This work was supported by grant numbers EY-06855 from the National Eye Institute/National Institutes of Health and R21 MH069688-01 from the National Institute of Mental Health/National Institutes of Health. The Government has certain rights in the invention.

FIELD OF THE INVENTION

The present invention relates generally to a hereditary ocular disorder, Collie Eye Anomaly (CEA), which affects development of the choroid and sclera in canines. More particularly, the invention relates to a method for identifying dogs as genetically normal, heterozygous for or homozygous for the CEA disease allele.

BACKGROUND OF THE INVENTION

Collie Eye Anomaly (CEA) is a canine hereditary ocular disorder affecting development of the choroid and sclera. The disease segregates in several dog breeds including Rough and Smooth Collies, Border Collies, Australian Shepherds, Lancashire Heelers, and Shetland Sheepdogs. The clinical phenotype varies significantly among affected dogs of all breeds. The primary CEA phenotype, choroidal hypoplasia (CH), is characterized by regional hypoplasia (underdevelopment) of the choroid, which is the highly vascularized bed of the eye that underlies the retina. This lesion usually results in an opthalmoscopically detectable window defect in the ocular fundus located temporal to the optic nerve.

In the most mildly affected dogs, CH is the only lesion apparent, and many such dogs will exhibit no obvious clinical consequences and retain apparently normal vision throughout life. In severely affected dogs, there may also be colobomatous lesions of the optic nerve head and or adjacent tissues. Colobomas are outpouchings of the eye wall, where there is localized thinness of the sclera. In the most severe cases, localized or complete retinal detachments, and/or intraocular neovascularization and hemmorrhage can develop, all of which can lead to blindness. These severe manifestations of CEA are only seen in dogs also affected with the primary choroidal hypoplastic lesion.

It has been previously established (Lowe J K, et al. Genomics 2003 July; 82(1):86-95) that the primary CEA phenotype is inherited via a gene that maps to a 3.9-cM region of canine chromosome 37, and segregates as an autosomal recessive trait with nearly 100% penetrance. However, because there has been no identification of an alteration of the gene associated with CEA, screening for the disease has not been possible. Thus, there has been an ongoing need in the canine breeding industry for a genetic test that permits direct identification of dogs that are normal, carriers or affected with CEA.

SUMMARY OF THE INVENTION

The present invention provides a method for identifying dogs which are genetically normal, heterozygous for or homozygous for the CEA disease allele. The method comprises the steps of obtaining a biological sample comprising genomic DNA from the dog and testing the biological sample for the presence or absence of a deletion of nucleotides corresponding to nucleotides from position 9,302 to position 17,101 of SEQ ID NO:1 within chromosome 37. The presence of the deletion in both alleles is indicative of a dog that is homozygous for the CEA disease allele. The presence of the deletion in only one allele is indicative of a dog that is heterozygous for the CEA disease allele, and the absence of the deletion in both alleles is indicative of a dog that is normal for CEA. The presence or absence of the deletion may be tested by amplification of the DNA followed by analysis of the amplification products.

The present invention also provides kits for diagnosis of a dog as normal, heterozygous for, or homozygous for the CEA disease allele. Such tools and/or kits assist breeders to identify normal dogs, carriers and homozygous mutant dogs. The dogs that are determined to be heterozygous for or homozygous for the disease allele can be eliminated from a breeding stock or bred with genetically normal dogs.

BRIEF DESCRIPTION OF THE DRAWINGS

FIG. 1 provides the sequence of SEQ ID NO:1 which corresponds to a region of chromosome 37 in dogs. SEQ ID NO:1 is a contig (a consensus sequence derived from multiple overlapping sequences) from nonaffected dogs. The area deleted in affected dogs and on one chromosome in dogs that are heterozygous for the CEA allele corresponds to nucleotides 9,302 to 17,101 of SEQ ID NO:1, which are indicated in lowercase. SEQ ID NO:1 corresponds to nucleotides 28,676,370 to 28,694,530, (inclusive, size 18,161 bp) of the public domain assembled canine genome sequence, July, 2004 Assembly, which can be accessed through GenBank or at the UCSC Genome Bioinformatics Site at genome.ucsc.edu/. SEQ ID NO:1 corresponds to nucleotides 72,769-90,929 of the Defined Collie Eye Anomaly Linkage Disequilibrium Interval. The Defined Collie Eye Anomaly Linkage Disequilibrium Interval corresponds to nucleotides 28,603,601 to 28,716,392 (inclusive, size 112,792 bp) of the public domain assembled canine genome sequence, July, 2004 Assembly. PCR primer binding sites are bolded and correspond to the primer names and positions listed in Tables 3-5. Sequences in lower case identify nucleotides deleted in the mutant allele; upper case identifies bases present in both normal and mutant.

FIG. 2 is a graphical representation of relative positions of the CEA deletion, SEQ ID NO:1, and primers used to test for the CEA deletion, in relationship to the CEA LD Interval, and in relation to positions in the assembled canine genome sequence (July, 2004 assembly). Relative to the coordinates of the canine genome sequence, both the sequence of the CEA deletion and of SEQ ID NO:1 are reversed.

FIG. 3A provides the nucleotide sequence (SEQ ID NO:10) corresponding to one strand of the amplification product obtained using primer CEAF21a and primer CEAR17d. The sequence corresponding to CEAF21a is bolded; the sequence corresponding to primer CEAR17d is underlined.

FIG. 3B provides the nucleotide sequence (SEQ ID NO:11) of the reverse complement of SEQ ID NO:10. The sequence corresponding to primer CEAF21a is bolded; the sequence corresponding to primer CEAR17d is underlined. The boxed pair of nucleotides “GC” flank the start breakpoint of the CEA deletion.

FIG. 4A provides the nucleotide sequence (SEQ ID NO:12) corresponding one strand of the amplification product obtained using primers CEAF22a and primer CEAR22c. The nucleotide sequence corresponding to primer CEAF22a is bolded; the sequence corresponding to primer CEAR22c is underlined.

FIG. 4B provides the nucleotide sequence (SEQ ID NO:13) of the reverse complement of SEQ ID NO:12. The nucleotide sequence corresponding to primer CEAF22a is bolded; the nucleotide sequence corresponding to primer CEAR22c is underlined. The boxed pair of nucleotides “GT” flank the end breakpoint of the CEA deletion.

FIG. 5 is a representation of an electrophoretic separation of PCR amplification products obtained using sets of the four PCR primers disclosed in Table 6. The first, leftmost, lane contains a size ladder. The remaining lanes are divided into four sets of PCR amplifications (1-4) of genomic DNA from normal (N), carrier (C) and affected (A) dogs. Set 1 was performed using primers CEAF22a and CEAR22c. Set 2 was performed using primers CEAF21a and CEAR22c. Set 3 was performed using primers CEAF21a and CEAR17d. Set 4 was performed using a combination of all four primers.

FIG. 6 provides the nucleotide sequence (SEQ ID NO:14) of one strand of the 430 bp product generated by PCR using primers CEAF21a and CEAR22c. The sequence corresponding to primer CEAF21a is bolded. The sequence corresponding to primer CEAT22c is underlined. The boxed nucleotides “GT” flank the deletion site.

DESCRIPTION OF THE INVENTION

The present invention is based on identification of the mutation associated with the CEA disease. We have reduced the critical region in which the CEA gene is located to an approximately 100 kb interval on chromosome 37 by using linkage disequilibrium mapping. Within this interval, a 7.8 kilobase (“kb”) deletion associated with dogs that are heterozygous for the deletion (carriers), or are homozygous for the deletion (likely to be affected with CEA), was identified. This 7.8 kb region is referred to herein as the “the CEA deletion.” Without intending to be bound by any particular theory, it is believed the CEA deletion results in removal or disruption of a putative enhancer element related to the expression of the CEA gene.

Disclosed in FIG. 1 is SEQ ID NO:1 which was assembled from data retrieved from The Institute for Genomic Research (TIGR) database of the preassembled 1.5× survey sequence database of the canine genome, together with sequences amplified and sequenced in the laboratory of Elaine Ostrander, by Dayna Akey. The contig created from this data formed the consensus sequence for SEQ: ID NO:1.

In more detail, SEQ ID NO:1 was assembled as a continuous 5′ to 3′ sequence in the direction of transcription of the putative gene FLJ12610 as part of an effort to identify the entire genomic sequence of this gene. The portion of FLJ12610 represented by SEQ ID NO:1 is presented in Table 1, with introns and exons also identified.

TABLE 1  1-519 End of Intron 1 of FLJ12610 520-732 Exon 2 of FLJ12610   733-8,053 Intron 3 of FLJ12610 8,054-8,191 Exon 3 of FLJ12610 8,192-8,781 Intron 3 of FLJ12610 8,782-8,840 Exon 4 of FLJ12610  8,841-18,160 Beginning of Intron 4 of FLJ12610  9,302-17,101 sequence deleted in CEA mutant allele

The gene FLJ12610 is transcribed from the reverse strand of canine chromosome 37, as it also is on the homologous human chromosome (HSA2). Thus, SEQ ID NO:1 runs forward in the same direction as the gene FLJ12610 is transcribed, but backwards in the canine genome assembly.

Table 2 shows the genomic positions of the Collie Eye Anomaly Linkage Disequilibrium Area, SEQ ID NO:1, and the Collie Eye Anomaly deletion. Nucleotide number 1 in SEQ ID NO:1 is the reverse complement of nucleotide 28,694,530 in the canine genome sequence, and the last nucleotide of SEQ ID NO:1 corresponds to the reverse complement of nucleotide 28,676,370 in the canine genome sequence. That is, SEQ ID NO:1 is the reverse complement of the interval 28,694,530 to 28,676,370 in the canine genome sequence.

TABLE 2 Feature Position on Canine Chromosome 37 Start LD 28,603,601 End SEQ ID NO: 1 28,676,370 End CEA Del 28,677,428 Start CEA Del 28,685,226 Start SEQ ID NO: 1 28,694,530 End LD 28,716,392

The breakpoints of the CEA deletion have also been identified. The CEA deleted region begins at nucleotide 9,302 of SEQ ID NO:1 which corresponds to nucleotide 28,677,428 of canine chromosome 37 of the public domain assembled canine genome sequence, July 2004 Assembly. Therefore the start breakpoint of the deletion (also referred to herein as the 5′ breakpoint) is between nucleotides 9,301 and 9,302 of SEQ ID NO:1. The deleted region ends at nucleotide 17,101 of SEQ ID NO:1 and therefore the end breakpoint of the deletion (also referred to herein as the 3′ breakpoint) is between nucleotides 17,101 and 17,102 of SEQ ID NO:1. When the CEA region is deleted, in a 5′ to 3′ sequence of the region corresponding to SEQ ID NO:1, nucleotide 9,301 (G) is followed by nucleotide 17,102 (T).

Based on the above observations, tests for detecting the presence or absence of the CEA deletion are provided. Dogs without the CEA deletion in either allele are referred to as normal for CEA. Dogs with the CEA deletion on only one allele are referred to as carriers of CEA. Dogs homozygous for the CEA deletions are referred to as affected with CEA.

Testing for the CEA deletion can be carried out in any sample which contains genomic DNA. For example, a sample of blood, hair, spleen, mucosal scrapings, semen, tissue biopsy, saliva or the like can be obtained. In one embodiment, the biological sample is blood.

The presence or absence of the CEA deletion may be determined using a variety of techniques that are well known in the art. For example, genomic DNA may be amplified for use in testing enzymatically through use of PCR (Saiki et al. Science 239:487-491 (1988)) or other in vitro amplification methods such as the ligase chain reaction (LCR) (Wu and Wallace Genomics 4:560-569 (1989)), strand displacement amplification (SDA) (Walker et al. PNAS USA 89:392-396 (1992)), self-sustained sequence replication (3SR) (Fahy et al. PCR Methods Appl. 1:25-33 (1992)), prior to CEA deletion analysis. Techniques for preparing nucleic acids in a form that is suitable for testing for the CEA deletion are well known in the art.

Detecting the presence or absence of the CEA deletion in DNA can be accomplished by a variety of methods including, but not limited to, polymerase chain reaction (PCR), fluorescent in situ hybridization (FISH), hybridization with allele-specific oligonucleotide probes (Wallace et al. Nucl Acids Res 6:3543-3557 (1978)), including immobilized oligonucleotides (Saiki et al. PNAS USA 86:6230-6234 (1989)) or oligonucleotide arrays (Maskos and Southern Nucl Acids Res 21:2269-2270 (1993)), allele-specific PCR (Newton et al. Nucl Acids Res 17:2503-25 16 (1989)), mismatch-repair detection (MRD) (Faham and Cox Genome Res 5:474-482 (1995)), denaturing-gradient gel electrophoresis (DGGE) (Fisher and Lerman et al. PNAS USA 80:1579-1583 (1983)), single-strand-conformation-polymorphism detection (Orita et al. Genomics 5:874-879 (1983)), chemical (Cotton et al. PNAS USA 85:4397-4401 (1988)) or enzymatic (Youil et al. PNAS USA 92:87-91 (1995)) cleavage of heteroduplex DNA, methods based on allele specific primer extension (Syvanen et al. Genomics 8:684-692 (1990)), genetic bit analysis (GBA) (Nikiforov et al. Nuci Acids Res 22:4167-4175 (1994)), the oligonucleotide-ligation assay (OLA) (Landegren et al. Science 241:1077 (1988)), the allele-specific ligation chain reaction (LCR) (Barrany PNAS USA 88:189-193 (1991)), gap-LCR (Abravaya et al. Nucl Acids Res 23:675-682 (1995)), and radioactive and/or fluorescent DNA sequencing using standard procedures well known in the art.

In one embodiment, amplification of genomic DNA for testing for the CEA deletion is performed by PCR. For this embodiment, PCR primers and a method of using the primers in amplification reactions are provided such that different combinations of amplification products are observed when DNA is amplified from affected, carrier or normal dogs.

In one embodiment, testing for the deletion is performed by PCR using a set of four primers. The primers are designed such that when the first and the second primers are used to amplify DNA from a normal chromosome 37 allele, a first amplification product is produced spanning the start breakpoint (5′ breakpoint) of the CEA deletion. The third and fourth primers are designed such that when they are used to amplify DNA from a normal chromosome 37 allele, a second amplification product is produced spanning the end breakpoint (3′ breakpoint) of the CEA deletion. The first and fourth primers are designed to bind to sites present adjacent to the area deleted in the disease chromosome. The second and third primers are designed to bind to sites present within the area deleted in the disease chromosome.

Neither the set of the first and second primers, nor the set of the third and fourth primers, will amplify a product from a chromosome 37 which has the CEA deletion because there is no binding site present for the second or third primers. Amplification using the first primer and the fourth primer will not produce an amplification product from a normal chromosome 37 because it is beyond the technical limitations of the amplification reactions employed herein to amplify and detect the 7.8 kb (undeleted) sequence present on the normal chromosome. However, when the CEA deletion is present, the binding sites for the first and fourth primers are placed in sufficient proximity with each other on the chromosome(s) with the CEA deletion such that a third amplification product is produced. Thus, the third amplification product does not contain any portion of the CEA deletion.

An example of a set of primers is provided wherein the first primer is upstream or 5′ of the start breakpoint of the CEA deletion and the second primer is within the CEA deletion but in sufficient proximity to the first primer site so that an amplification product can be produced spanning the start breakpoint of the CEA deletion. The third primer is within the CEA deletion and the fourth primer is downstream or 3′ of the end breakpoint of the CEA deletion. The third and the fourth primer are in sufficient proximity such that an amplification product is produced spanning the end breakpoint of the CEA deletion. The first and the fourth primer sites are sufficiently apart so that when the CEA region is not deleted, these two primers will not produce any amplification product.

It will be recognized by those skilled in the art that the primer designations as first, second, third and fourth is arbitrary and is used herein for clarity in reference to the amplification products generated using the particular primer pairs. It will also be recognized that, while particular sequences of PCR primers are provided herein, other PCR primer sequences can be designed by those skilled in the art to detect the presence or absence of the CEA deletion. Further, the primers may be designed to amplify either strand of chromosome 37 in the region of the CEA deletion.

Amplification reactions can be carried out using all four primers in the same reaction or amplification of each set can be carried out separately. Thus, simultaneous or sequential amplifications of the genomic DNA in separate reactions using the first and second primers, the third and fourth primers, and the first and fourth primers can also be performed. Regardless of whether the amplifications are performed separately or in combination, the combined results of the amplifications using the three aforementioned primer pairs are interpreted as follows:

1) The presence of only the first and second amplification products is indicative of a normal dog.

2) The presence of the first, second and third amplification products is indicative of a carrier dog.

3) The presence of only the third amplification product is indicative of an affected dog.

Thus, by using the combination of primer pairs described herein, the PCR amplification product profile obtained from a biological sample indicates the CEA status of the dog as normal, a carrier or affected.

When PCR primers are used such that the amplification products are of distinct sizes, the amplification products can be analyzed by standard methods such as electrophoretic separation and detection using ethidium bromide and ultraviolet light, or any other suitable detection method. Alternatively, the PCR products can be isolated and sequenced.

The method of the present invention can be carried out for any breed of dog. In general, dogs known to be inflicted by CEA include Rough and Smooth Collies, Border Collies, Australian Shepherds, Lancashire Heelers, and Shetland Sheepdogs.

Also provided in the present invention are kits for detecting the presence of the CEA deletion in a biological sample from a dog or a nucleic acid sample extracted from the biological sample. The kits of the present invention comprise reagents for nucleic acid based detection of the presence of the CEA deletion. In one embodiment, the kits comprise reagents for extraction/preparation of nucleic acid samples, pairs of primers for amplification of regions spanning the start breakpoint and end breakpoint of the CEA deletion and pairs of primers for amplification of a region spanning the region generated by deletion of the CEA region.

By using the tools and method described herein, dogs which are genetically normal, heterozygous for (deletion in one allele), or homozygous for (deletion in both alleles) the mutation primarily responsible for Collie eye anomaly (CEA) can be identified. Upon identification, such dogs can be eliminated from a breeding stock. Alternatively, dogs which are heterozygous for the CEA allele can be mated with genetically normal dogs to ensure the absence in the litter of dogs affected with CEA.

The invention will be further understood by the following examples, which are intended to be illustrative and not restrictive in any way.

Example 1

This example demonstrates that dogs which are genetically normal, heterozygous for, or homozygous for the mutation primarily responsible for CEA can be distinguished using the method of the present invention. In particular, combinations of four primers are used in PCR reactions to produce amplification products characteristic of dogs that are genetically normal, heterozygous for, or homozygous for the mutation primarily responsible for CEA. The binding positions of the primers relative to SEQ ID NO:1, the CEA deletion and the CEA linkage disequilibrium interval (LD) are provided in FIG. 2.

FIG. 3A provides the nucleotide sequence (SEQ ID NO:10) corresponding to one strand of the amplification product obtained using primer CEAF21a and primer CEAR17d. FIG. 3B provides the nucleotide sequence (SEQ ID NO:11) of the reverse complement of SEQ ID NO:10. In the reverse complement, the boxed pair of nucleotides “GC” flank the start breakpoint of the CEA deletion. That is, on the reverse strand of CFA (Canis familias) chromosome 37 the G is not deleted, but the C is the first deleted nucleotide in the mutant allele. Table 3 provides additional information about the relative binding positions of primers CEAF21a and CEAR17d.

TABLE 3 Primer CEAF21a CEAR17d Sequence GGAGGAGTCATCATGACTTGC GACTGGTATTATCAAAGGTCAC (SEQ ID NO:2) (SEQ ID NO:4) Reverse GCAAGTCATGATGACTCCTCC GTGACCTTTGATAATACCAGTC Complement (SEQ ID NO:3) (SEQ ID NO:5) of Sequence Binding site GGAGGAGTCATCATGACTTGC gtgacctttgataataccagtc sequence, in (SEQ ID NO:2) (SEQ ID NO:5) SEQ ID NO:1 Location 9213-9233 9495-9474 relative to SEQ ID NO:1 Location −89 to −69 +194 to +173 relative to START of CEA deletion Location chr37:28,685,296-28,685,315 chr37:28,685,033-28,685,054 relative to Assembled Canine Genome Sequence

FIG. 4A provides the nucleotide sequence (SEQ ID NO:12) corresponding to one strand of an amplification product obtained using primers CEAF22a and primer CEAR22c. FIG. 4B (SEQ ID NO:13) provides the reverse complement of SEQ ID NO:12. In the reverse complement, the boxed pair of nucleotides “GT” flank the end breakpoint of the CEA deletion. That is, on the reverse strand of CFA 37, the G is the last deleted nucleotide and the T is not deleted in the mutant allele. Table 4 provides additional information about the relative binding sites of primers CEAF22a and CEAR22c.

TABLE 4 Primer CEAF22a CEAR22c Sequence TGTCCTCCGTACCATCGTGT CTAGTCTGTCAATAGCACCACTA (forward) (SEQ ID NO:6) (SEQ ID NO:8) Reverse ACACGATGGTACGGAGGACA TAGTGGTGCTATTGACAGACTAG Complement (SEQ ID NO:7) (SEQ ID NO:9) of Sequence Binding site TGTCCTCCGTACCATCGTGT TAGTGGTGCTATTGACAGACTAG sequence, in (SEQ ID NO:6) (SEQ ID NO:9) SEQ ID NO:1 Location 16739-16758 17420-17442 relative to SEQ ID NO:1 Location −363 to −344 +341 to +319 relative to END of CEA deletion. Location chr37:28,677,770-28,677,789 chr37:28677088-28677110 relative to Assembled Canine Genome sequence

To distinguish CEA affected, carrier and normal dogs, the primers disclosed in Table 3 and 4 (and which are summarized in Table 5) were used as follows.

TABLE 5 Primer Sequence Binding Site Location CEAF21a GGAGGAGTCATCATGACTTGC GGAGGAGTCATCATGACTTGC 9213- (SEQ ID NO:2) (SEQ ID NO:2) 9233 CEAR17d GACTGGTATTATCAAAGGTCAC gtgacctttgataataccagt 9474- (SEQ ID NO:4) (SEQ ID NO:5) 9493 CEAF22a TGTCCTCCGTACCATCGTGT tgtcctccgtaccatcgtgt 16739- (SEQ ID NO:6) (SEQ ID NO:6) 16760 CEAR22c CTAGTCTGTCAATAGCACCACTA TAGTGGTGCTATTGACAGACTAG 17420- (SEQ ID NO:8) (SEQ ID NO:9) 17442

CEAF21a is a forward primer and designated herein as a first primer, CEAR17d is a reverse primer and is designated herein as a second primer. CEAF22a is a forward primer and is designated herein as a third primer and CEAR22c is a reverse primer and is designated herein as a fourth primer. Three sets of primers for PCR tests as depicted in Table 6 (“PCR Test #” and “Primers” columns) were performed. These sets of primers were used to amplify genomic DNA extracted from canine blood samples by the phenol-chloroform method (Sambrook et al. 1989). In initial studies, DNA was used from 3 selected dogs whose CEA genetic status (affected, normal or carrier; “CEA Status” column) had been previously determined by experimental breeding studies. In subsequent studies, DNA was used on a larger set of samples representing more than 20 dogs of each genotype (affected, normal or carrier), for which the genotype that had been previously established by experimental breeding studies. All amplifications used the same PCR program: 96° C. for 2 minutes; 30 cycles of 96° C. (20 seconds), 58° C. (20 seconds), and 72° C. (40 seconds); and a final extension at 72° C. for 5 minutes. PCR products were analyzed by eletrophoresis through a 1.5% agarose gel (FIG. 5). The assignment of phenotypes was based on the presence or absence of particular size PCR products as listed in the “Expected PCR Product” column. PCR test number 4 used all four primers simultaneously.

TABLE 6 Expected PCR Test # Primers CEA Status Product 1 CEAF22a Affected None CEAR22c Normal 704 bp Carrier 704 bp 2 CEAF21a Affected 430 bp CEAR22c Normal None Carrier 430 bp 3 CEAF21a Affected None CEAR17d Normal 283 bp Carrier 283 bp 4 CEAF22a Affected 430 bp CEAR17d Normal 283 bp CEAF21a 704 bp CEAR22c Carrier 283 bp 430 bp 704 bp

As shown in Table 6 and FIG. 5, for CEA test 1 (primers CEAF22a and CEAR22c) no product is amplified from affected (A), but a 704 bp product is amplified from both Normal (N) and Carrier (C). This result is obtained because, in the N and C samples, there is at least one copy of the normal CEA allele on which the CEAF22a and CEAR22c primer binding sites are separated by 704 base pairs (bp). However, the CEAF22a binding site lies within the region of DNA that is deleted from both alleles in the affected animals, thus there is no binding site for CEAF22a present on the mutant chromosome and no amplification product can be detected. The sequences of each strand of the 704 bp product generated by PCR using primers CEAF22a and CEAR22c is disclosed in FIGS. 4A and 4B.

As shown in FIG. 5, for CEA test 2 (primers CEAF21a and CEAR22c) a 430 bp product is amplified from both affected (A) and carrier (C), but no product is amplified from Normal (N). This result is obtained because, in both affected and carrier dogs, there is at least one allele with the CEA deletion. The deletion juxtaposes the CEAF21a and CEAR22c primer binding sites such that they are separated by 430 bp on the mutant allele. However, in the normal allele (no PCR product observed), the CEAF21a and CEAR22c primer binding sites are over 7,800 bases apart. Thus, the theoretical product from normal DNA is too large to be amplified and/or observed under the described testing conditions using the CEAF21a and CEAR22c primers. The sequence of one strand of the 430 bp product (SEQ ID NO:14) generated by PCR using primers CEAF21a and CEAR22c is provided in FIG. 6 wherein the boxed nucleotides “GT” are juxtaposed due to the deletion.

As shown in FIG. 5, for CEA test 3 (primers CEAF21a and CEAR17d), no product is amplified from affected (A), but a 283 bp product is amplified from both Normal (N) and Carrier (C). This result is obtained because, in the N and C samples, there is at least one copy of the normal CEA allele, and the CEAF21a and CEAR17d primer binding sites are separated on the normal allele by 283 bp. However, the CEAR17d binding site lies within the region of DNA that is deleted from both alleles in the affected phenotype, thus there is no binding site for CEAR17d and no amplification product can be detected. The sequence of both strands of the 283 bp product generated by PCR using primers CEAF21a and CEAR17d is disclosed in FIGS. 3A and 3B. Subsequent tests have confirmed that the indicated length of the 283 bp product is correct despite its apparent migration as a longer product in FIG. 5.

In CEA test 4, all primers for tests 1 through 3 are multiplexed, with each of the attendant PCR products produced as when the tests are performed with the single sets 1-3. As can be seen from test 4, only one product (430 bp) is amplified from affected (A), while a 283 bp and a 704 bp product are amplified from Normal (N); and all 3 products (283, 430, and 704 bp) are amplified from the Carrier (C) sample when all four primers are used.

Thus, this Example demonstrates that, by using the method of the present invention, dogs that are normal at the CEA locus, or are heterozygous for, or are homozygous for CEA mutation can be identified.

While this invention has been illustrated by specific embodiments, routine modifications will be apparent to those skilled in the art and such modifications are intended to be within the scope of the invention and the following claims. 

1. A kit for identifying a dog as normal, heterozygous for, or homozygous for a Collie Eye Anomaly mutation in a region of chromosome 37, wherein the mutation consists of a deletion of nucleotides 9,302 to 17,101 of SEQ ID NO:1, comprising: a set of primers, wherein the only primers in the kit are a first primer, a second primer, a third primer and a fourth primer, wherein the first primer, the second primer, the third primer, and the fourth primer each consist of a fragment of SEQ ID NO:1 or the complement thereof, wherein the first primer binds to a sequence upstream of position 9,301 of SEQ ID NO:1, the fourth primer binds to a sequence downstream of position 17,102 of SEQ ID NO:1 and second and third primers binds to a sequence between nucleotides 9,302 and 17,101 of SEQ ID NO:1, wherein amplification of an allele that does not comprise the mutation with the first and the second primers produces a first amplification product that comprises the nucleotide 9,302 of SEQ ID NO:1, amplification of an allele that does not comprise the mutation using the third and fourth primers produces a second amplification product that comprises the nucleotide 17,101 of SEQ ID NO:1, and amplification using the first and the fourth primer produces a third amplification product, wherein the third amplification product comprises SEQ ID NO:14 or a fragment thereof wherein the fragment thereof comprises contiguous nucleotides 89 and 90 of SEQ ID NO:14.
 2. The kit of claim 1, wherein the first primer has the sequence of SEQ ID NO:2, the second primer has the sequence of SEQ ID NO:4, the third primer has the sequence of SEQ ID NO:6 and the fourth primer has the sequence of SEQ ID NO:8. 